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US2905677A - Counter current extraction process of sterols - Google Patents

Counter current extraction process of sterols Download PDF

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US2905677A
US2905677A US656609A US65660957A US2905677A US 2905677 A US2905677 A US 2905677A US 656609 A US656609 A US 656609A US 65660957 A US65660957 A US 65660957A US 2905677 A US2905677 A US 2905677A
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stigmasterol
stages
solvent
stripping
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Glen A Fevig
John W Greiner
Kenneth W Riebe
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Pharmacia and Upjohn Co
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Upjohn Co
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    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D11/00Solvent extraction
    • B01D11/02Solvent extraction of solids
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07JSTEROIDS
    • C07J75/00Processes for the preparation of steroids in general

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  • This invention relates to a novel process for the countercurrent fractional separation of crude mixtures of sterols. It relates more particularly to improvements in the countercurrent selective solvent separation of natural mixtures of sterols, which mixtures may contain tarry materials and other naturally occurring impurities which may or may not be chemically or physically modified, in addition to the sterols.
  • Figure 1 illustrates three cycles of the process of the invention in diagrammatic fashion.
  • Figure 2 shows a single cycle in a process in accordance with the invention.
  • Figure 3 illustrates diagrammatically a practical embodiment of the invention.
  • Natural sterol mixtures occur as residues in the refining of natural oils and waxes, usually occurring as a mixture of two or more sterols possessing molecular structural differences which may vary from profound to slight.
  • the crude sterol mixtures also contain in most instances coloring matter and other materials, regarded, for the purpose of this invention, as impurities.
  • sterols such as stigmasterol and ergosterol are useful as starting materials in the synthesis of steroid compounds that possess great pharmacological value. Owing to the aforesaid differences in sterol structure, it is necessary to accomplish the desired steroid synthesis in a manner that is dependent upon the structure of the individual sterol starting materials, and it is therefore necessary to start with a sterol of high purity.
  • One of the important sterols currently useful as a starting material in making steroid compounds of great pharmacological value is stigmasterol, occurring as a lesser constitutent in crude soy sterols, the major constituents of soy sterols being sitosterols.
  • the starting mixtures for the process of the present invention are solid mixtures consisting essentially of stigmasterol and sitosterols (plus impurities such as those already noted). stigmasterol and the sitosterols commonly occur together as mixtures obtained from various natural sources, e.g., from soybeans as previously .mentioned, sugar cane, calabar and coffee beans, etc. Stigmasterol ordinarily comprises only from about five to about 35 percent of the total crude sterols from these sources, the remainder being mostly sitosterols.
  • One of the aspects of this invention is the provision of improvements in the countercurrent separation of stigmasterol from mixtures of sterols containing sitosterols as well as other sterols, and the aforesaid impurities in minor amounts.
  • stigmasterol or other selected desired sterol is recovered as a leached or crystallized product of high purity by a separation method which comprises a series of countercurrent selective solvent separations in which the starting sterol mixture travels through a series of enriching stages to the final purified end product.
  • Solvents simultaneously travel through the enriching stages in reverse order, and continue through a series of stripping stages to a final stage wherein all the constituents of the original sterol mixture except the desired sterol are held in solution, and a precipitated cake passes forward sequentially through the stripping stages eventually to join the feed solids travelling through the enriching stages.
  • a stripping stage to be elfective in accomplishing a separation, results in a precipitated sterol product having a different composition compared with the sterols still held in solution. The difference results in either an enriched or depleted content of the desired sterol in the precipitated sterol cake.
  • the enriched precipitated cake can be passed through the enriching stages, or in the latter case the enriched mother liquor can be treated to recover the dissolved solids, and those solids, being enriched in the desired sterols, can be passed through the enriching stages.
  • FIG. 1 illustrates three cycles of such a process as described above, employing five enriching stages and two stripping stages in each cycle.
  • the enriching stages are shown as squares and the stripping stages are shown as circles.
  • Each portion of the starting mixture is shown as F, the feed solids.
  • the first enriching stage is shown as S in the drawing and the fifth as S
  • a stripping stage according to this invention involves the separation (stripping) from the mother liquor of a portion of the solids dissolved therein, obtained from one of the preceding stripping stages or the first enrich ing stage (feed stage).
  • the process illustrated in Figure 1 represents two stripping stages, the first employing the mother liquor obtained from the first enriching stage of that cycle and the second employing the mother liquor obtained from the first stripping stage.
  • the first stripping stage of each cycle is shown as S in the drawing and the second as S A cycle refers herein to a segment of a countercurrent extraction wherein a portion of the starting mixture, ,enriched in stigmasterol, is obtained at one end of the system as undissolved solids, and the portion depleted .in stigmasterol, dissolved in the spent solvent, is obtained at the other end.
  • the stages of the first cycle are shown third cycle, C
  • soysterols as the sterol mixture and stigmasterol as the desired sterol
  • soysterols as the sterol mixture
  • stigmasterol as the desired sterol
  • This a value is determined experimentally by partially dissolving the sterol mixture, e.g., a mixture of stigmasterol and sitosterols such as crude soy sterols, in an organic solvent, as described above, and then determining the stigmasterol and sitosterols content of the dissolved and of the undissolved solids.
  • the ,8 value of the solvent for that particular mixture and solvent-solid ratio can be determined by the following formula:
  • whcreinS is the stigmasterol content (percent) of the undissolved solids (cake)
  • NS is thenon-stigmasterol (sitosterols) content (percent) of the undissolved solids (by difference)
  • NS is the non-stigmasterol content (percent) of-the dissolved solids in the motherliquor- (by difference)
  • Sm is the stigrnasterol'content (percent) ofthe dissolved solids.
  • the solvents employed in the process of-the present invention are-those selective organic solvents having a relative distribution coefficient greater than 1.5 at a volume of solvent which dissolves about one-half of the total solids of a sample of the sterol mixture employed as starting mixture in-the process. These solvents are capable of producing a final product of high stigmasterol content efficiently and economically.
  • the selective organic solvent employed in the process of the present invention be readily available and reasonably inexpensive, be noncorrosive to equipment, be chemically inert to ster'ols, possess a high solvent power for sterols, present no difiicultymanageable safety problems such as fire, explosion, and toxicity, and possess long-term stability in order to permit repeated recycling, reclaiming, and reusing.
  • the data required for determining B value are conveniently obtained as follows, employing a stigmasterolsitosterols mixture and a volume of the organic solvent which at room temperature dissolves approximately onehalf of the sterols mixture, as already stated in the foregoing.
  • the sterols-solvent slurry is brought to equilibrium, preferably by vigorous agitation for at least one-half hour at temperatures between about twenty and about 35 degrees centigrade.
  • equilibration can be achieved by heating the slurry to a sufficiently hightemperature to dissolve the sterols, slowly coolingthe resulting solution, with stirring, to between about twenty and about 35'degrees Centigrade, and maintaining the resulting slurry at substantially the same reduced temperature conditions for at least one-half hour.
  • the solid phase (cake or undissolved solids) and the liquid phase (mother liquor containing dissolved. solids) of the equilibrated slurry are separated by conventional means, such as filtration, or centrifugation.
  • the cake is dried and its. stigmasterol content is determined by assay, e.g., infrared assay; the non-stigmasterol (sitosterols) content is determined by diiference.
  • the dissolved solids of the mother liquor are isolated by evaporating the mother liquor. to dryness and the stigmasterol content of the dry residue is determined by assay, e.g., infrared assay; the nonstigmasterol (sitosterols) content .is determined by difference.
  • the ,8 value of the solvent, for the particular mixture and solvent-solid ratio is conveniently calculated in accordance with the preceding formula.
  • Preferred organic solvents are those selective organic solvents which are carbon compounds having from one to eight carbon atoms, inclusive, and which have at least one additional element selected from the group consisting of hydrogen, oxygen, chlorine and bromine; which are liquids at ordinary temperatures and pressures, and which have relative distribution coefiicients (5 values) greater than 1.5.
  • solvents-include lower aliphatic hydrocarbons such as n-pentane, n-hexane, n-heptane, SkellysolveB (essentially amixtureof hexanes), Skellysolve C (essentially, a mixture of hexanes and heptanes), petroleum ether, isoo'ctane, cyclohexane, methylcyclohexane, l-pentene, 1*-octene, and the like; halogenated lower aliphatic hydrocarbons, such as ethylene dichloride, methylene chloride, propylene chloride, chloroform, ethylene dibromide, tetrachloroethylene, carbon tetrachloride, and the like; mixtures of lower aliphatic hydrocarbons and halogenated lower.
  • lower aliphatic hydrocarbons such as n-pentane, n-hexane, n-heptane, Skelly
  • aliphatic hydrocarbons such as fifty ercent n-heptane-fifty percent ethylene dichloride mixture by volume, or the n-heptane-ethylene dichloride azeo-f trope, consisting of approximately 37' percentn-heptane and 63 percent ethylene dichloride by volume, and the like; lower aromatic hydrocarbons, such as benzene, tolue ene, xylene, and the like; lower-aliphatic ketones, such as acetone, methyl isobutylketone, and the like; lower aliphatic alcohols, such as ethanol, isobutyl alcohol, nbutyl alcohol, n-propyl-alcohol, n-amyl alcohol, Z-methoxyethanol, '2-ethoxyet'hanol, o-methylcyclohexanol, and the.
  • lower aromatic hydrocarbons such as benzene, tolue ene, xylene, and the like
  • halogenated lower aromatic hydrocarbons such as chlorobenzene, bromob'enzene, o-dichlorobenzene, and the like
  • halogenated lower aromatic hydrocarbons such as chlorobenzene, bromob'enzene, o-dichlorobenzene, and the like
  • - lower aliphatic ethers such as diisopropyl ether, dioxa'ne,'and the like
  • lower aliphatic esters such as ethyl acetate, amyl acetate, ethyl butyrate, and the like.
  • lower aliphatic hydrocarbons and halogenated lower aliphatic hydrocarbons are preferred, especially ethylene dichloride: and n heptane, and mixturesthereof,particularlytheir azeotropic mixture having, as already noted, a composition of approximately37 percent' n heptane and 63'percent ethylene dichloride'by volume.
  • soy 'sterols'together withthe extracting solvent, i. e. leaching 'on crystallizing solvent, are placedin a r 5 container and made into a slurry.
  • the slurry is agitated for a period of time until equilibrium is reached.
  • the soy sterols are completely dissolved in the solvent, advantageously with the aid of heat, and the resulting solution is cooled and equilibrated to precipitate a portion of the sterol solids.
  • the mother liquor is separated from undissolved solids by filtration, and the cake is placed in a ditferent container together with fresh solvent.
  • the filtrate containing dissolved stigmasterol, sitosterol and other materials, is freed of some of its dissolved sterols by the stripping operation, i.e., precipitation or crystallization of dissolved sterols. This can be accomplished by reducing the temperature, distilling oft some of the solvent, or by other known methods. Separation of the resulting mixture into a mother liquor and a cake is then carried out.
  • a batchwise countercurrent separation process has the advantage of permitting carefully controlled conditions of time of contact, ratio of solvent to solids, efiicient mechanical separation of the solids from the filtrate, etc. to be employed. After selecting the optimum solvent, volume of solvent, temperature, time, number of stages, etc., to produce the desired purity of stigmasterol in' the first cycle of operation, these conditions can be maintained in successive cycles during the countercurrent operation, giving reasonable assurance of a product of controlled purity, or the conditions can be varied as may be desired.
  • the batchwise countercurrent separation process that characterizes the present invention usually involves at least four enriching stages per cycle and ordinarily, at least five. Six enriching stages, when employing a reasonably efficient solvent, are ordinarily sufiicient to achieve the production of very high purity stigmasterol.
  • the primary advantage offered by a stripping stage is that it permits a higher yield of the desired sterol, i.e., stigmasterol, per cycle.
  • the number of stripping stages is usually less than the number of enriching stages. Generally speaking, if the number of stripping stages per cycle is increased, using any given selective solvent, the yield increases.
  • the stripping stages have a profound effect upon the overall yield because efiicient stripping tends to direct previously dissolved stigmasterol toward the enriching end of the cycle. Without eflicient stripping, most of the stigmasterol that is dissolved in stage 1 would appear in the solvent residue.
  • this drawing represents a single cycle in a process such as characterizes this inven tion. Portions of the preceding and succeeding cycles are shown in dotted lines. The arrows indicate for each stage the streams which enter and leave. Arrows slanting to the right represent the path of separated solids, while those slanting to the left represent the path of the filtrates.
  • the stability of a continuing process and its ability to produce consistently high yields of high quality material involve careful control of the ratio of the desired sterol in the cakes to that in the filtrates from which they are separated, i.e., the E value. This stability can best be achieved by a routine pilot determination of E,
  • stage 1 the sterol feed, and the stage 0 cake (from the preceding cycle), are slurried with stage 2 filtrate (from the preceding cycle) and make-up fresh solvent.
  • 1 slurry,- is; filteredat. the. predetermined. temperature to. yeaun vame. dff japproxiinately. 1.2 to 1.7.
  • the resulting filtrate is passed to the succeeding cycle, and'thecake, is reslurriedin stage 4 filtrate (from the precedingcycle) to make up stage 3.
  • the procedure is followed flthroughthe remainder of'the cycle as shownin Figurelup to stage 6, where the stage 5 cake is reslurriecLin freshsolvent.
  • stage 6 cake i.e., the final stigmasterol product
  • the stage 6 cake is removed from the filter press anddried, and the'stage 6 filtrate is used subsequently to, reslurry the stage;,4- cake, thusto make up stage 5 in the succeeding cycle.
  • the filtrate, obtained instage 1' is mixed with the cake from stage -1 of the. preceding cycle.
  • the resulting stage 0 slurry is heated to dissolve the solids, distilled toremove water andito adjust the solids concentration; the solution is then cooled to an intermediate holding temperature, the calculated amount of water is added and dissolved therein, the solution is further cooled to crystallization temperature, andis finally filtered.
  • the cakefrom stage 0 is sent to stage 1 of the succeeding cycle and the filtrate is passed to stage 1 oflthein'stant cyclewhere it receives and is mixed with the cake from stake 2 of, the preceding cycle and is stripped according to the procedure described above for the stage 0 slurry.
  • Sta s ,2 is carriedv out substantially the same as stage 0, and stage l, described above, using the cake from stage, -3 of the preceding cycle and the filtrate from stage-l of the instant cycle.
  • Stage -3 is carried out in a manner similar to the above, but using only stage -2 filtrate. of the instant cycle, and the resulting mother liquor, i.e., stage 3 filtrate, leaves the processa's a residue.
  • the solvents involved in the process of countercurrent separation described herein frequently contain minor amounts, of water, up to, say, 0.05 percent of water by volume. This minor amount of water must besupplemented by additional amounts, in order to realize the beneficial efiect on 3 value, according to this invention.
  • each of' the stripping stages shown in Figure 2 the entry of water is shown by a vertical arrow.
  • the stripping. can becarried out over a broad range of temperature, i.e., from'about minus twenty degrees centigrade to plus thirty degrees centigrade or higher.
  • Concentration of total solids'in stripping stage slurries broadl'y lies within the range of ten to thirty percent by weight,.the said total solids including suspended solids as-wellas dissolved solids. In stages 0 and 2 the concentrationis advantageously in the, range of twenty to thirty percent,;and in stage l, in the, range, of ten to twenty percent.
  • E the ratio. of: HOB? stigmasterol materials, in the cake to that in.the filtrate
  • the ratio of E to E is the fl-value for a given separation. This valueis, a function of. the starting mixture in any stage and. the; solvent used in that stage. It can be varied somewhat: by varying the temperature and concentration, but onthe whole it is a property of a mixture over which the operator has little control in production operation with. a given. solvent-solids. system.
  • C-lOoJilMM 108 (Iii/IF) (stigmasterol) 1 can be removed simply and easily by distillation, i.e., as a ternary azeotrope (when the extracting solvent used in the process is the n-heptane-ethylene dichloride azeotrope previously mentioned). After removal of water,-
  • the resulting dried filtrate is used in stage 1 to dissolve wherein n is the base-11h? tTfih$1111S1PI1 (P at 970 the stripped cake from stage 2; the resulting solution and IP is the actual fl'ahsmlssloh (P at 970 is then stripped using added water to increase selectivity cmr C 18 the percent stigmasterol content of the unof stripping, d h resulting k i passed t stage 0 known sample. of the succeeding cycle.
  • the filtrate is passed to the next Once a countercurrent separat on 18 1n operatlon ut1l1zt i i Stage, L Stage 2, i h a System as Shown ing the process of our invent1on, 1t 1s unnecessary to make i Fi 2, superfluous or repetitive determinanons of ,3 value, s1nce I a system employing b t t stripping stages, th then only rout1ne checks are neededfiltrate from stage 1 is, of course, the residue.
  • the filtrate from the 1116 followlng data 1n Table I illustrate the var1at1ons 1n preceding stripping stage, e g,, stage 2, is concentrated 1 Value as effe cted y the q h 0f Wat61 added duflng to a substantially reduced volume by distillation.
  • stage 86 1 the e value begins to drop at about three moles of added water per mole of stigrnasterol present.
  • stage 0 the e value begins to drop at about three moles of added water per mole of stigrnasterol present.
  • stage 0 the e value begins to drop at about three moles of added water per mole of stigrnasterol present.
  • stage 0 the e value begins to drop at about three moles of added water per mole of stigrnasterol present.
  • stage 0 the eflect of adding increasing amounts of water in begins to drop at about the same range of added water.
  • stage -1 is shown in Table II.
  • Table IV below shows the effect of added water on TABLE II Stage Stripping stage data-Stage -1 TABLE IV Stripping stage data-Sttzge 2 H 0 wt Cake W ⁇ : .dot Solfifldts essay, s01 s in add edI cake, perpent in filt., assay, E. E 8 H2O Wt g gf f 5 5 9 added cake, percetit in filt., assay, E. E,, 5
  • gm. stig. gm. percent stig. is 32 iii 33 35 2:05 810 113 26:1 49 0171 0129 2.' 47 a? Moles of H20 added per mole of stigmasterol present. i Moles of H20 added per mole of stigmasteml present It can be Seen from Tabl? H that the effect of addihg In Table IV above it can be seen that as the range of t 8 amounts of Water In Stage 1 affords a defimhe added water reaches above 8.0 moles per mole of stighh the 1 Value to a maxlmhm, Whereafter addl' I masterol present, the addition of further water has little tlonal amounts of water cause the ,8 value to decrease.
  • stage data-Stage 1 TABLE v V 5 Stripping. stage data-Stage 1..
  • Figure 3 showing a practical embodiment of the invention by means of a flow diagram.
  • the squares of the drawing represent stages in which slurries are (a) prepared, (b) equilibrated, and (c) filtered.
  • a horizontal line of squares will. be referred to as a row.
  • the drawing illustrates two rows in a plant operation which consists of six enriching stages and four. stripping stages per cycle.
  • arrows slanting to the left represent liquid streams,,i.e;,.filtrates proceeding from one stage (stage.n.)-to another stage (stage n 1) except-in the case of by-pass which will be explained in detail below.
  • stage 3 the arrow slanting to the left represents the residue filtrate which, leaves the process.
  • Leftward slanting arrows also show the addition of fresh solvent where needed in the process.
  • Arrows pointing vertically upward represent thejrejmovalsofliquidfrom the process by distillation. This. removal is carried out for thepurpose of removing water by ,azeotopic distillation and for the further purpose of adjusting. the solids concentration in any givenstage to that required for the purposeof the stage, for example, stripping, astigmasterol-enriched cake from the-solution.
  • stage 6 Set up stage 6 of next row by pumping the slurry to stage tank, heating to dissolve all the solids, and cool to crystallize preparatory to filtration.
  • stage 6 a preliminary laboratory filtration is carried out, and E 12 E and flvalues are determined. Theternperature, is then, adjusted prior. to filtration. in order, to getlhe E value.
  • stage 4 of the next row by pumping the slurryt to a stage tank, adding three hundred gallons of 3 fresh solvent, dissolving the slurried solids by heating, coolingto crystallize, performing preliminary laboratory filtration; etc. as with the stage above.
  • stage 2 Set up stage 2 of the next row by pumping the slurry.- to a stage tank, dissolving, crystallizing, etc. asabover FILTER STAGE -1 AND SET'UP'STAGE" 0 OF NEXT ROW a. Pump stage 1 filtrateto the filter cake receiver.
  • stage 2 Set up stage 2 by'distilling, preliminary cooling, adding water, and further cooling, as in stage 0'.
  • the above operations complete the filtration steps of the upper row of stages, leaving the lower row of stagesto be filtered.
  • the lower row is treated as follows.
  • FILTER STAGE G (NO SET UP) a. Filter a major proportion of stage 6 onthefiltcl'. press; dry the cake as stigmasterol product. Leave the1 remainder of the slurry unfiltered in the stage tank, to be used as reflux to stage 5 of the succeeding row.
  • stage -2 filtrate to stage tank.
  • b Strip as described for stage 0.
  • the foregoing illustrative procedure is taken from a large-scale process for separating stigmasterol from a feed of mixed soy sterols, the entire process having been operated a sufiiciently long time so that steady state conditions prevail.
  • the stigmasterol product is of extremely high quality, the yield is very high, and the stigmasterol content of the process residue is very low.
  • the efficiency of stripping contributes materially to the two latter features, i.e., high overall yield of stigmasterol product and low stigmasterol content of the residue.
  • stage 3 to stage 1 by-pass by manipulation such as described above, delays the production of stigmasterol product of 90.8 percent average quality, using six enriching stages and two stripping stages, with an overall stigmasterol yield of 65.3 percent.
  • production of 90.1 percent quality stigmasterol product requires eight enriching stages and two stripping stages with an overall yield of 52.4 percent.
  • by-passing stage 3 to 1 it is likewise feasible as noted above to by-pass stage 4 to stage 2, stage 2 to stage 0, or stage 1 to stage -1.
  • the two stages involved in the by-passing of a particular filtrate can be determined by observing the quality of materials moving through the system.
  • the by-pass points are selected so as to obviate mixingstreams containing sterols having markedly unequal stigmasterol content. It is feasible moreover to by-pass the filtrate around more than one stage, if necessary, to combine it with a cake of similar stigmasterol content.
  • a process for the separation and purification of stigmasterol and sitosterols by the extraction of sito-' sterols from a starting solid stigmasterol and sitosterols mixture consisting essentially of stigmasterol and sitosterols which comprises contacting the starting solid stigmasterol and sitosterols mixture with a selective organic solvent having the following characteristics; 1) a greater solvent aflinity for the siteosterols as determined on a test portion of said starting solid stigmasterol and sitosterols mixture by employing a volume of the organic solvent which dissolves approximately one-half of the solids of the test portion of the said starting solid stigmasterol and sitosterols mixture, and (2) a relative distribution coeflicient (18) in said test greater than 1.5, said relative distribution coefficient (5) being determined according to the formula:
  • S is the stigmasterol content in percent of the undissolved solids
  • NS is the non-stigmasterol content in percent of the undissolved solids (by difference)
  • S is the stigmasterol content in percent of the dissolved solids in the mother liquor
  • NS is the non-stigmasterol content in percent of the dissolved solids in the mother liquor (by difference)
  • stigmasterol said solutions and said stripped cakes -travel-.
  • 2,-..Th8..process of claiml wherein the amountofiwater added is from, about. 2 to about. 3 moles, per. molevofstigmasterol in the first stripping stage, from about ⁇ . to.
  • tGIOlS which comprises. contacting the starting solid stigmasterol and sitosterols mixture with a selective organic solvent having the following characteristics; (1) a greater solvent affinity. for the sitosterols asdetermined on..a. test portion of said starting solid stigmasterol and.
  • sitosterols mixture by employing a volume of the organic solvent which dissolves approximately one-half of the. solidsof the test portion of the said starting, solid stigmasterol and sitosterols mixture, and.( 2)- a relative distribution coefiicient (B) in said test. greater than; 1.5,

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Description

Sept. 22, 1959 G. A. FEVIG ETAL 2,905,677
COUNTER CURRENT EXTRACTION PROCESS OF STEROLS Filed May 2, 1957 3 Sheets-Sheet 1 .ld, ar
s LEGEND i [:l ENRICHING STAGE STRIPPING STAGE FFEED souos FIGURE P UNDISSOLVED souos GLEN A FEVIG ESH SQLv JOHN w. GREINER --MOTHER LIQUOR KENNETH W RIEBE c CYCLE v I INVENTOR. s= STAGE 1 Maw! P= PRODUCT BY 6 041064,,
A TTORNEY Sept. 22, 1959 COUNTER CURRENT EXTRACTION PROCESS OF STEROLS Filed May 2, 1957 3 Sheets-Sheet 2 ESIDUE a: GLEN A. FEVIG JOHN W. GREINER KENNETH W. RlEBE INVENTOR.
A TTORNE Y United States Patent COUNTER CURRENT EXTRACTION PROCESS OF STEROLS Glen A. Fevig, Kalamazoo, John W. Greiner, Kalamazoo Township, Kalamazoo County, and Kenneth W. Riebe, Kalamazoo, MiclL, assignors to The Upjohn Company, Kalamazoo, Mich., a corporation of Michigan Application May 2, 1957, Serial No. 656,609
Claims. (Cl. 260-39725) This invention relates to a novel process for the countercurrent fractional separation of crude mixtures of sterols. It relates more particularly to improvements in the countercurrent selective solvent separation of natural mixtures of sterols, which mixtures may contain tarry materials and other naturally occurring impurities which may or may not be chemically or physically modified, in addition to the sterols.
Figure 1 illustrates three cycles of the process of the invention in diagrammatic fashion. Figure 2 shows a single cycle in a process in accordance with the invention. Figure 3 illustrates diagrammatically a practical embodiment of the invention.
Natural sterol mixtures occur as residues in the refining of natural oils and waxes, usually occurring as a mixture of two or more sterols possessing molecular structural differences which may vary from profound to slight. In addition to the sterols, the crude sterol mixtures also contain in most instances coloring matter and other materials, regarded, for the purpose of this invention, as impurities.
Many sterols such as stigmasterol and ergosterol are useful as starting materials in the synthesis of steroid compounds that possess great pharmacological value. Owing to the aforesaid differences in sterol structure, it is necessary to accomplish the desired steroid synthesis in a manner that is dependent upon the structure of the individual sterol starting materials, and it is therefore necessary to start with a sterol of high purity. One of the important sterols currently useful as a starting material in making steroid compounds of great pharmacological value is stigmasterol, occurring as a lesser constitutent in crude soy sterols, the major constituents of soy sterols being sitosterols.
The starting mixtures for the process of the present invention are solid mixtures consisting essentially of stigmasterol and sitosterols (plus impurities such as those already noted). stigmasterol and the sitosterols commonly occur together as mixtures obtained from various natural sources, e.g., from soybeans as previously .mentioned, sugar cane, calabar and coffee beans, etc. Stigmasterol ordinarily comprises only from about five to about 35 percent of the total crude sterols from these sources, the remainder being mostly sitosterols.
One of the aspects of this invention is the provision of improvements in the countercurrent separation of stigmasterol from mixtures of sterols containing sitosterols as well as other sterols, and the aforesaid impurities in minor amounts.
According to this invention in its broad aspect, stigmasterol or other selected desired sterol is recovered as a leached or crystallized product of high purity by a separation method which comprises a series of countercurrent selective solvent separations in which the starting sterol mixture travels through a series of enriching stages to the final purified end product. Solvents simultaneously travel through the enriching stages in reverse order, and continue through a series of stripping stages to a final stage wherein all the constituents of the original sterol mixture except the desired sterol are held in solution, and a precipitated cake passes forward sequentially through the stripping stages eventually to join the feed solids travelling through the enriching stages.
The present invention relates especially to the stripping stages, and involves methods for increasing the efficiency of the stripping operation. This operation, in order .to give the best effective and practical overall results, must afford the removal of solids richer in the desired sterol than the total dissolved solids in the unstripped solu-. tion. Successive stripping stages should ultimately lead to a final residual solution that is sufiiciently low in dissolved desired sterol as to be economically suitable as a process residue.
Broadly speaking, a stripping stage, to be elfective in accomplishing a separation, results in a precipitated sterol product having a different composition compared with the sterols still held in solution. The difference results in either an enriched or depleted content of the desired sterol in the precipitated sterol cake. It can be seen that in the former case the enriched precipitated cake can be passed through the enriching stages, or in the latter case the enriched mother liquor can be treated to recover the dissolved solids, and those solids, being enriched in the desired sterols, can be passed through the enriching stages. In practice we have found it preferable to carry out the stripping so that the stripped solids, enriched in the desired sterol (e.g., stigmasterol), are obtained directly as a cake and the cake passed directly through the enriching stages. This avoids the engineering complications of separating from enriched mother liquor sterols the highly soluble impurities contained therein.
Reference is made to Figure 1 of the accompanying drawings which illustrates three cycles of such a process as described above, employing five enriching stages and two stripping stages in each cycle. In Figure 1 the enriching stages are shown as squares and the stripping stages are shown as circles. Each portion of the starting mixture is shown as F, the feed solids.
An enriching stage is a point in the process where a selective solvent separation is conducted, i.e., the chosen solvent is mixed with the sterol solids to partially dissolve these solids by leaching, or the sterol solids are completely dissolved in the chosen solvent and the resulting solution is cooled and equilibrated, to precipitate a portion of the sterol solids enriched in stigmasterol; and the undissolved solids, enriched in stigmasterol, are then separated from the solvent and dissolved solids (filtrate). The first enriching stage is shown as S in the drawing and the fifth as S A stripping stage according to this invention involves the separation (stripping) from the mother liquor of a portion of the solids dissolved therein, obtained from one of the preceding stripping stages or the first enrich ing stage (feed stage). The process illustrated in Figure 1 represents two stripping stages, the first employing the mother liquor obtained from the first enriching stage of that cycle and the second employing the mother liquor obtained from the first stripping stage. The first stripping stage of each cycle is shown as S in the drawing and the second as S A cycle refers herein to a segment of a countercurrent extraction wherein a portion of the starting mixture, ,enriched in stigmasterol, is obtained at one end of the system as undissolved solids, and the portion depleted .in stigmasterol, dissolved in the spent solvent, is obtained at the other end. The stages of the first cycle are shown third cycle, C
stripping stage of the second cycle as C 8 the second stripping stage of the third cycle as C 8 etc.
Solvents employed in the process of the present invention are selective organic solvents having a greater solvent aflinity for. the residual sterols, i;e., sitosterols, determined on a portion of the starting sterol mixture to be used in the countercurrent leaching (or crystallization) process, employing a volume of the organic solvent which dissolves approximately one-half of the solids (e.g., forty to. sixty percent) of the portion of the sterol mixture tested.
For. a clear understanding of the following description, addressing attention illustratively to soysterols as the sterol mixture and stigmasterol as the desired sterol, the-ensuing definitions of symbols are given.
weight 'of stigmasterol in the oalte Weight of stigmasterol in tli'filtrat'e' This symbol (E is a measure of the stigmasterol dissolved in, any one stage.
Weigh of nonstigmasterol-materialsin the cal e weight of non-stigrnasterol materials in the filtrate symbol (En) is a measure of the non-stigmasterol materialsdissolved in any one stage.
E. (weight of stigmasterol in the cake) E (weight of non-sti masterol materialsin the cake) (weight of non-stigrnasterol materials in the filtrate) (weight, of non-stigmasterol in the filtrate This symbol, the 13 value, is the relative distribution coefiic ient of'the solvent (used in that stage) and varies with the, solvent-solid ratio and with the ratio of stigmasterol to nonestigmasterol materials that characterizes the solid. It is a measure of the degree of selectivity of a selective organic solvent.
This a value is determined experimentally by partially dissolving the sterol mixture, e.g., a mixture of stigmasterol and sitosterols such as crude soy sterols, in an organic solvent, as described above, and then determining the stigmasterol and sitosterols content of the dissolved and of the undissolved solids. The ,8 value of the solvent for that particular mixture and solvent-solid ratio, can be determined by the following formula:
whcreinS is the stigmasterol content (percent) of the undissolved solids (cake), NS is thenon-stigmasterol (sitosterols) content (percent) of the undissolved solids (by difference), NS is the non-stigmasterol content (percent) of-the dissolved solids in the motherliquor- (by difference) and Sm is the stigrnasterol'content (percent) ofthe dissolved solids. i
If the relative distribution coeflicientof an organic solvent is greater than 1.0 for a mixture of stigmasterol andsitosterols at a particular volume of solvent, then that vorganic solvent-produces undissolved solids of enriched stigmasterol content overthe original mixture. Thesolvents employed in the process of-the present invention are-those selective organic solvents having a relative distribution coefficient greater than 1.5 at a volume of solvent which dissolves about one-half of the total solids of a sample of the sterol mixture employed as starting mixture in-the process. These solvents are capable of producing a final product of high stigmasterol content efficiently and economically. It is likewise desirable, for economic and operating reasons, that the selective organic solvent employed in the process of the present invention be readily available and reasonably inexpensive, be noncorrosive to equipment, be chemically inert to ster'ols, possess a high solvent power for sterols, present no difiicultymanageable safety problems such as fire, explosion, and toxicity, and possess long-term stability in order to permit repeated recycling, reclaiming, and reusing.
The data required for determining B value are conveniently obtained as follows, employing a stigmasterolsitosterols mixture and a volume of the organic solvent which at room temperature dissolves approximately onehalf of the sterols mixture, as already stated in the foregoing. The sterols-solvent slurry is brought to equilibrium, preferably by vigorous agitation for at least one-half hour at temperatures between about twenty and about 35 degrees centigrade. Alternatively, equilibration can be achieved by heating the slurry to a sufficiently hightemperature to dissolve the sterols, slowly coolingthe resulting solution, with stirring, to between about twenty and about 35'degrees Centigrade, and maintaining the resulting slurry at substantially the same reduced temperature conditions for at least one-half hour. The solid phase (cake or undissolved solids) and the liquid phase (mother liquor containing dissolved. solids) of the equilibrated slurry are separated by conventional means, such as filtration, or centrifugation. The cake is dried and its. stigmasterol content is determined by assay, e.g., infrared assay; the non-stigmasterol (sitosterols) content is determined by diiference. The dissolved solids of the mother liquor are isolated by evaporating the mother liquor. to dryness and the stigmasterol content of the dry residue is determined by assay, e.g., infrared assay; the nonstigmasterol (sitosterols) content .is determined by difference. With these data at hand the ,8 value of the solvent, for the particular mixture and solvent-solid ratio, is conveniently calculated in accordance with the preceding formula.
Preferred organic solventsare those selective organic solvents which are carbon compounds having from one to eight carbon atoms, inclusive, and which have at least one additional element selected from the group consisting of hydrogen, oxygen, chlorine and bromine; which are liquids at ordinary temperatures and pressures, and which have relative distribution coefiicients (5 values) greater than 1.5. Representative solvents-include lower aliphatic hydrocarbons, such as n-pentane, n-hexane, n-heptane, SkellysolveB (essentially amixtureof hexanes), Skellysolve C (essentially, a mixture of hexanes and heptanes), petroleum ether, isoo'ctane, cyclohexane, methylcyclohexane, l-pentene, 1*-octene, and the like; halogenated lower aliphatic hydrocarbons, such as ethylene dichloride, methylene chloride, propylene chloride, chloroform, ethylene dibromide, tetrachloroethylene, carbon tetrachloride, and the like; mixtures of lower aliphatic hydrocarbons and halogenated lower. aliphatic hydrocarbons, such as fifty ercent n-heptane-fifty percent ethylene dichloride mixture by volume, or the n-heptane-ethylene dichloride azeo-f trope, consisting of approximately 37' percentn-heptane and 63 percent ethylene dichloride by volume, and the like; lower aromatic hydrocarbons, such as benzene, tolue ene, xylene, and the like; lower-aliphatic ketones, such as acetone, methyl isobutylketone, and the like; lower aliphatic alcohols, such as ethanol, isobutyl alcohol, nbutyl alcohol, n-propyl-alcohol, n-amyl alcohol, Z-methoxyethanol, '2-ethoxyet'hanol, o-methylcyclohexanol, and the. like; halogenated lower aromatic hydrocarbons, such as chlorobenzene, bromob'enzene, o-dichlorobenzene, and the like;- lower aliphatic ethers, such as diisopropyl ether, dioxa'ne,'and the like; and lower aliphatic esters, such as ethyl acetate, amyl acetate, ethyl butyrate, and the like. Of these solvents, lower aliphatic hydrocarbons and halogenated lower aliphatic hydrocarbons are preferred, especially ethylene dichloride: and n heptane, and mixturesthereof,particularlytheir azeotropic mixture having, as already noted, a composition of approximately37 percent' n heptane and 63'percent ethylene dichloride'by volume. I
fln 'carrying outan illustrative embodiment ofthis iiivention, soy 'sterols'together withthe extracting solvent, i. e. leaching 'on crystallizing solvent, are placedin a r 5 container and made into a slurry. The slurry is agitated for a period of time until equilibrium is reached. Alternatively, the soy sterols are completely dissolved in the solvent, advantageously with the aid of heat, and the resulting solution is cooled and equilibrated to precipitate a portion of the sterol solids. At the end of this period the mother liquor is separated from undissolved solids by filtration, and the cake is placed in a ditferent container together with fresh solvent. The filtrate, containing dissolved stigmasterol, sitosterol and other materials, is freed of some of its dissolved sterols by the stripping operation, i.e., precipitation or crystallization of dissolved sterols. This can be accomplished by reducing the temperature, distilling oft some of the solvent, or by other known methods. Separation of the resulting mixture into a mother liquor and a cake is then carried out.
The cake from the original separation (stage 1 cake) is treated with fresh solvent to provide a second cake (stage 2 cake) and a second mother liquor (stage 2 filtrate). The stage 2 filtrate together with fresh make-11p solvent is used to treat a combined feed consisting of fresh feed sterol and the cake (stage cake) from the preceding stripping stage. Referring to Figure 1, it can be seen that upon eventual attainment of steady state conditions, a true batchwise countercurrent process has been developed.
A batchwise countercurrent separation process has the advantage of permitting carefully controlled conditions of time of contact, ratio of solvent to solids, efiicient mechanical separation of the solids from the filtrate, etc. to be employed. After selecting the optimum solvent, volume of solvent, temperature, time, number of stages, etc., to produce the desired purity of stigmasterol in' the first cycle of operation, these conditions can be maintained in successive cycles during the countercurrent operation, giving reasonable assurance of a product of controlled purity, or the conditions can be varied as may be desired.
The batchwise countercurrent separation process that characterizes the present invention usually involves at least four enriching stages per cycle and ordinarily, at least five. Six enriching stages, when employing a reasonably efficient solvent, are ordinarily sufiicient to achieve the production of very high purity stigmasterol.
In a batchwise countercurrent separation process, desirable results are obtained when at least four enriching stages per cycle are employed and when the separation is performed in a manner such that, in the slurry produced in these stages, more than fifty percent of the stigmasterol remains undissolved (E l). An E value of 1.2-3.0 is a satisfactory normal operating range and advantageous results are obtained if E is between 1.2 and 6.0, e.g., if between about 55 and 85 percent of the stigmasterol remains undissolved in these stages, all of which can be accomplished by temperature and solvent volume adjustment as will be readily apparent to one skilled in the art. In addition, especially advantageous quality product is obtained if the ratio of undissolved to dissolved stigmasterol in these stages is maintained at least 1.5 times the ratio of undissolved to dissolved sitosterols, which attends the use in these stages of a solvent having a relatively high ,8 value, i.e., above 1.5.
In following the process as described above, we have discovered a surprisingly efiective method for improving the efliciency of the separation, especially in the stripping stages and in the early enriching stages, i.e., stage 1 and stage 2. Ideally, stripping should accomplish the precipitation only of the desired sterol, hence necessitating but one stripping stage; but this is not attainable in practice. Though enrichment of the desired sterol, i.e., stigmasterol, in the stripped cake can be accomplished by a wide variety of methods, all conventional methods known to us are of such a character that they cannot easily be integrated into the overall countercurrent system. It can be readily seen, however, that the selective removal of stigmasterol in the stripping stages is highly" desirable because of the resulting improvement in overall yield of stigmasterol from the starting sterol mixture.
The primary advantage offered by a stripping stage is that it permits a higher yield of the desired sterol, i.e., stigmasterol, per cycle. The number of stripping stages is usually less than the number of enriching stages. Generally speaking, if the number of stripping stages per cycle is increased, using any given selective solvent, the yield increases. The stripping stages have a profound effect upon the overall yield because efiicient stripping tends to direct previously dissolved stigmasterol toward the enriching end of the cycle. Without eflicient stripping, most of the stigmasterol that is dissolved in stage 1 would appear in the solvent residue.
Stripping can be accomplished by means of adding materials such as precipitants to the filtrates in the stripping stages but in most instances this introduces a variety of complicating factors. For example, solvent recoveries are complicated, and the possibility always exists that the succeeding enriching stages will be thrown out of balance by the presence of added substances in the solvent system, that is, such substances are passed from stage to stage. We have discovered that the presence of water can and does in most instances produce an undesirable etfect in the enriching stages of the process, particularly those stages occurring after the second enriching stage. Sterols, including stigmasterol and sitosterols, tend to form solvates with water, and the solubilities of these solids in the solvents are thus greatly altered. We have discovered, on the other hand, that the presence of water in carefully controlled amounts in the stripping stages and early enriching stages aids in the separation of stigmasterol from non-stigmasterol material.
We have discovered that the surprising and desirable effect of water in controlled amounts in this process is an improved separation of stigmasterol from non-stigmasterol materials, i.e., a decreased affinity of the solvent for stigmasterol. This occurs optimally when the total sterols present in any stage consist of not more than onefourth stigmasterol by weight. This ordinarily involves the early enriching stages, i.e., stages 1 and 2, and the stripping stages, as previously mentioned. We have found that if too much water is used, this effect is lost.
We have further found that if too little water is used, the desirable effect is diminished or sometimes not achieved.
Referring now to Figure 2, this drawing represents a single cycle in a process such as characterizes this inven tion. Portions of the preceding and succeeding cycles are shown in dotted lines. The arrows indicate for each stage the streams which enter and leave. Arrows slanting to the right represent the path of separated solids, while those slanting to the left represent the path of the filtrates.
The cycles which follow are identical to the one shown with respect to the how pattern. Each square in the drawing represents a stage in which the operations of slurrying, equilibration and filtration, are carried out successively. In practice, filtrations are conveniently carried out in the order, 6, 4, 2, 0, 2, 5, 3, 1, l, 3, whereupon the cycle is completed and the next one begins 6, 4, etc.
The stability of a continuing process and its ability to produce consistently high yields of high quality material involve careful control of the ratio of the desired sterol in the cakes to that in the filtrates from which they are separated, i.e., the E value. This stability can best be achieved by a routine pilot determination of E,,
value at a given temperature for a given slurry, and then' adjusting the temperature of the main slurry prior to filtration so that the desired E value is achieved. In stage 1, the sterol feed, and the stage 0 cake (from the preceding cycle), are slurried with stage 2 filtrate (from the preceding cycle) and make-up fresh solvent. The
1 slurry,- is; filteredat. the. predetermined. temperature to. yeaun vame. dff japproxiinately. 1.2 to 1.7.
Thezsiage, 1. cakeis reslurriedriri stage. 3 filtrate (from theprecedingcycle) and fresh make-up solvent, to make up stage2, andthe filtration is, carried out as above. The resulting filtrate is passed to the succeeding cycle, and'thecake, is reslurriedin stage 4 filtrate (from the precedingcycle) to make up stage 3. The procedure is followed flthroughthe remainder of'the cycle as shownin Figurelup to stage 6, where the stage 5 cake is reslurriecLin freshsolvent. The stage 6 cake, i.e., the final stigmasterol product, is removed from the filter press anddried, and the'stage 6 filtrate is used subsequently to, reslurry the stage;,4- cake, thusto make up stage 5 in the succeeding cycle.
The different filtratesfromthis cycle are held in storage; as is necessary to their use in the succeeding cycles. Theaboye operations have been described in the order oftheir occurrence in the cycle. The chronological orderfofi the, steps. that is actually followed is set forth above.
The filtrate, obtained instage 1' is mixed with the cake from stage -1 of the. preceding cycle. The resulting stage 0 slurry is heated to dissolve the solids, distilled toremove water andito adjust the solids concentration; the solution is then cooled to an intermediate holding temperature, the calculated amount of water is added and dissolved therein, the solution is further cooled to crystallization temperature, andis finally filtered. After filnation, the cakefrom stage 0, is sent to stage 1 of the succeeding cycle and the filtrate is passed to stage 1 oflthein'stant cyclewhere it receives and is mixed with the cake from stake 2 of, the preceding cycle and is stripped according to the procedure described above for the stage 0 slurry.
Sta s ,2, is carriedv out substantially the same as stage 0, and stage l, described above, using the cake from stage, -3 of the preceding cycle and the filtrate from stage-l of the instant cycle. Stage -3 is carried out in a manner similar to the above, but using only stage -2 filtrate. of the instant cycle, and the resulting mother liquor, i.e., stage 3 filtrate, leaves the processa's a residue.
The solvents involved in the process of countercurrent separation described herein frequently contain minor amounts, of water, up to, say, 0.05 percent of water by volume. This minor amount of water must besupplemented by additional amounts, in order to realize the beneficial efiect on 3 value, according to this invention.
In each of' the stripping stages shown in Figure 2, the entry of water is shown by a vertical arrow. The quantity of water added inthese stages, as well as in the early enriching stages in accordance with thisinvention, lies in the range of 0.5 to twelve, preferably 0.5 to ten, moles of water per mole of stigmasterol. It is advantageously in the range of 0.5 to four moles in stage 0. Advant'ageously, it broadens slightly in stage -l where the range can be about one to live. Slightly more water can be added advantageously in stage 2, i.e., two to seven moles of water per mole or stigmasterol. As additional stripping stages are added, the molar ratio of water to stigmasterol' in the additional stages can be gradually increased.
The stripping. can becarried out over a broad range of temperature, i.e., from'about minus twenty degrees centigrade to plus thirty degrees centigrade or higher. Concentration of total solids'in stripping stage slurries broadl'y lies within the range of ten to thirty percent by weight,.the said total solids including suspended solids as-wellas dissolved solids. In stages 0 and 2 the concentrationis advantageously in the, range of twenty to thirty percent,;and in stage l, in the, range, of ten to twenty percent.
one ofthe important features of the overall process which characterizesthis invention is the proper regulationof the E valueat each stage. In generahthevalue. of E shouldbe greater than 1.0 in the strippingand en-r riehing stages. Thevalue of E (the ratio. of: HOB? stigmasterol materials, in the cake to that in.the filtrate) should in general be less than 1.0. The ratio of E to E is the fl-value for a given separation. This valueis, a function of. the starting mixture in any stage and. the; solvent used in that stage. It can be varied somewhat: by varying the temperature and concentration, but onthe whole it is a property of a mixture over which the operator has little control in production operation with. a given. solvent-solids. system. Thus, one could-achieve ahigh yield of stigmasterol by using a high E valu'e. at every stage but the [3 value relationship would cause, the E values also to be high, and a low quality product; would tend to result. On the other hand, the use of E values, while assuring a good quality product, would result in low yields. The small variations in the 5 value that are possibleby manipulating the temperature; and concentration in practical plant operations do not alter appreciably this end result.
Onthe other hand, when it is possible as in this inven-' tion to introduce a new factor, i.e., alter the character of thesolvent and thus'increase the p value at will, then it is possible to increase the yield and the quality of. product.
In a system of countercurrent separation operations for separating a desired sterol from undesired sterols as:- sociated in solution by selective precipitation of the;- former, i.e., by selective stripping, it is hencedesirable; to increase the ,3 value of thesystemwhere:
(weight of stigmasterol stripped from solution) (weight of non-stigmasterol materials stripped from solution) X (weightofstigmasterol remaining insolution) As described above, it is a feature of this invention to add controlled amounts of water to the solution in such stripping stages and in the early enriching stages; and this feature of our invention is based upon our discovery that the 13 value will be increased as a result. The amount of water added to increase the 3 value in aparticular embodiment of our invention has been described above as'falling within specified ranges. In systerns employing a diiferent number of stripping stages, different solvents, or different sterol mixtures, the range of amounts of water effective to increase the 5 value in" accordance with this invention can readily be ascertained merely by a series of routine tests adding gradu ated amounts of water and determining the 18 value from theformula:
B cX ml m! given above.
Methods are known for determining quantitatively the stigmasterol content in a mixture of sterols. On method. for determining stigmasterol in admixture withsitosterols is by infrared spectrum analysis as follows. The sample. is dissolved, at a precise concentration of 50.0 milli: grams per milliliter, in chloroform and the spectrumof; this solution is. recorded from 930 cm.- to 1025, cm? in a double beam spectrophotometer which gives at least percent transmission at 970 cm.- when both the sample and reference cells are filled with chloroform. alone. The cells are approximately 0.5 millimeter thick; A sample of pure stigmasterol is spectroanalyzed in exact-: ly the same manner. 0n the records of, the absorption pattern of both the unknown sample and the stigmasterol, a base-line having a slope of 0.2, is;drawn from.the peak.
C-lOoJilMM 108 (Iii/IF) (stigmasterol) 1 can be removed simply and easily by distillation, i.e., as a ternary azeotrope (when the extracting solvent used in the process is the n-heptane-ethylene dichloride azeotrope previously mentioned). After removal of water,-
the resulting dried filtrate is used in stage 1 to dissolve wherein n is the base-11h? tTfih$1111S1PI1 (P at 970 the stripped cake from stage 2; the resulting solution and IP is the actual fl'ahsmlssloh (P at 970 is then stripped using added water to increase selectivity cmr C 18 the percent stigmasterol content of the unof stripping, d h resulting k i passed t stage 0 known sample. of the succeeding cycle. The filtrate is passed to the next Once a countercurrent separat on 18 1n operatlon ut1l1zt i i Stage, L Stage 2, i h a System as Shown ing the process of our invent1on, 1t 1s unnecessary to make i Fi 2, superfluous or repetitive determinanons of ,3 value, s1nce I a system employing b t t stripping stages, th then only rout1ne checks are neededfiltrate from stage 1 is, of course, the residue. In the Employlhg as Stage 0 feed a f g 1 filtrate from a final stripping stage of a system employing four stripping stlgmasterql p g y system e as Shown m F g 2 stages, e.g., stage -3 of Figure 2, the filtrate from the 1116 followlng data 1n Table I illustrate the var1at1ons 1n preceding stripping stage, e g,, stage 2, is concentrated 1 Value as effe cted y the q h 0f Wat61 added duflng to a substantially reduced volume by distillation. This Stage 0 pp d glvell In Tables I through process removes the water previously added and provides, V were obtamed using mIXed S Y St61'0l t a Solvent, therefore, a dried solution containing the dissolved solids the azeotrope 9f n-heptane and e yl dwhlonde; the of the stage -2 filtrate. When a reduction in volume is same applies to the data set forth In Flgure 3. reached which is suitable for the final stripping operation,
In Table I, the da a a gro p aCCOIdlIlg t0 h Stage this operation is carried out as previously described. The 0 feed- In each group It can be Seen that the addltlon of cake is passed to the succeeding cycle and the filtrate rewater caused an increase in the ,8 value. The table also c vered s a process re idue, illustrates roughly var1ations in ,8 value that result from Table III further illustrates the effects on the B value changes 1n temperature and feed materlal. of adding gradually increasing amounts of water in TABLEI stage S I d S 0 TABLE III In m sta e atata e pp 8 g g Strzppzng stage data-StageO Stage 0 H2O Cryst. Feed, Cake Wt. of Solids 0ono.gm.sollds/ added, temp., E. E8 5 percent, H2O Wt. assay, solids in fllt.
. gm. slurry percent C. stigmasadded cake, percent in tllt., assay, E. E 6
by vol. terol by gm. stig. gm. percent LR. stig.
a... M0 1687 35 at 34 hi it is 33 3 1 1 Q67 1:13: 2511 1718 288 912 1169 0179 2124 so. 15 w W itt- 34 526 i3 is 45 016 i 1:89: 3717 1713 22:8 514 5.30 1: 45 3165 0 0 0.74 0.48 1.53 13.6 2.64. 41.5 14.6 18.1 6.0 5.56 2.08 2.67 0 0 0.43 0.38 1.14 13.6 3.40. 44.9 14.3 14.4 7.1 6.28 2.88 2.18
{ 4 1. 0 0 28 092 3.04 1&6 4.15 45.7 13.9 12.9 8.8 5.61 3.35 1.68
{ 1 1 g 0 25 31 77 6 1 Moles of H20 added per mole of stigmasterol present.
{ 0,10 m 1 81 0 58 3 12 14.2 Referrlng back to Table II, 1t can be seen that at stage 86 1 the e value begins to drop at about three moles of added water per mole of stigrnasterol present. The same M0193 0f H4O added Per 0f stlgmasterh Present effect is shown for stage 0 in Table III where the ,8 value The eflect of adding increasing amounts of water in begins to drop at about the same range of added water. stage -1 is shown in Table II. Table IV below shows the effect of added water on TABLE II Stage Stripping stage data-Stage -1 TABLE IV Stripping stage data-Sttzge 2 H 0 wt Cake W{: .dot Solfifldts essay, s01 s in add edI cake, perpent in filt., assay, E. E 8 H2O Wt g gf f 5 5 9 added cake, percetit in filt., assay, E. E,, 5
gm. stig. gm. percent stig. is 32 iii 33 35 2:05 810 113 26:1 49 0171 0129 2.' 47 a? Moles of H20 added per mole of stigmasterol present. i Moles of H20 added per mole of stigmasteml present It can be Seen from Tabl? H that the effect of addihg In Table IV above it can be seen that as the range of t 8 amounts of Water In Stage 1 affords a defimhe added water reaches above 8.0 moles per mole of stighh the 1 Value to a maxlmhm, Whereafter addl' I masterol present, the addition of further water has little tlonal amounts of water cause the ,8 value to decrease. ff t upon the 5 value 'P h fofegolllgi It can be Seen f the Process of Table V below shows the effect of adding water in stage the mvemwn provldes e q by whlqh the fi l 1. This table illustrates that our invention is applicable can be controlled, In p h Increased, 111 the strlpplhg to the early enrichingstages as disclosed above, i.e., stages. stages. The water added 1n stage 0, for example, part 1 and 2, as well as the stripping stages. It can be seen of which'carries over in the filtrate that is passed to stage from Table V that the optimum amount of added water appears 1'1 is,.r eached at slightlyrrnorethan two molesof waterper, mole of stigmasterol present,.and that atabout five molest of-waterxpermole of stigmasterol present. the. valueshowsanettdecrease in value.
TABLE v V 5 Stripping. stage data-Stage 1..
, Cake Wt. of Solids H2O Wt. assay, solids in filt. adde cake, percent in filt., assay, E; En 43 gm. stig. gm. percent stig.
47. 3 26;? 51. 2 13.7 1. 78 0. 81 2. 2 77. 2, 23. 5 70. 3 12. 6 2. 05 0; 96 2. 13 77. 1 23. 7 69. 0 13. 7, l. 93 ll. 99 1. 95 15 37. 3' 24. 7 35. 0 12. 3 2:14 0. 92 2. 34 38. 2 26. 2 33. 9 7. 5 3. 94 0. 9O 4. 38 56. 3. 20. 2 9.7 8. 5 13. 8 5. 06 2. 73 4. 71 24. 3' 51. l 16. l 1.39 0. 83 1. 67
'Moles-ct 1110 added per mole of stigmasterol present.
Reference is made toFigure 3 showing a practical embodiment of the invention by means of a flow diagram. The squares of the drawing represent stages in which slurries are (a) prepared, (b) equilibrated, and (c) filtered. A horizontal line of squares will. be referred to as a row. The drawing illustrates two rows in a plant operation which consists of six enriching stages and four. stripping stages per cycle.
In the drawing, arrows slanting to the left represent liquid streams,,i.e;,.filtrates proceeding from one stage (stage.n.)-to another stage (stage n 1) except-in the case of by-pass which will be explained in detail below. In stage 3 the arrow slanting to the left represents the residue filtrate which, leaves the process. Leftward slanting arrows also show the addition of fresh solvent where needed in the process.
Arrows slanting to the right represent. the flow offilter. cakes proceeding from a stage (stage n) to a succeed: ing stage (stage n+l). In stage 6 the arrow-slanting to the right represents, the final stigmasterol productof the process.
Arrows pointing vertically upward represent thejrejmovalsofliquidfrom the process by distillation. This. removal is carried out for thepurpose of removing water by ,azeotopic distillation and for the further purpose of adjusting. the solids concentration in any givenstage to that required for the purposeof the stage, for example, stripping, astigmasterol-enriched cake from the-solution.
Arrows pointing vertically downward represent water added in the stripping stages. Insome of the stages, water is added to solutions already containing an appreciable amount of water; so the amount indicated as added does not represent the total effective amount present. The arrow pointing vertically downward in stage 1 represents feed soy sterols that are added. The fractions adjacent to the slanting arrows which represent the liquid and solid streams, and also the fractions contained in the squares representing stages, are the weight ratios of stigmasterol to the solids present. The percentage figures also represent these ratios. The volume of slurry in-a stage prior to filtration is shown below the stage square. Thesequential operations beginning with the step of filtrationfor the top row of stages are as follows, the term set up as used herein being substantially synonymous with the word prepare.
FILTER STAGE E AND SET UP STAGE 6 OF NEXT ROW a.v Pump one thou sand gallons of fresh solvent into filter cake receiver.
b. Filter stage 5, reslurrying the cake in the solvent in filter cake receiver.
c.v Set up stage 6 of next row by pumping the slurry to stage tank, heating to dissolve all the solids, and cool to crystallize preparatory to filtration. In this stage, a preliminary laboratory filtration is carried out, and E 12 E and flvalues are determined. Theternperature, is then, adjusted prior. to filtration. in order, to getlhe E value.
FILTERVVSTAGE 3 AND SET UP STAGE 4 OF NEXT ROW.
a. Pump stage 5 filtrate to the filter cake receivers;
b. Filter stage. 3, receiving the cake in the staged; filtrate.
0. Set up stage 4 of the next row by pumping the slurryt to a stage tank, adding three hundred gallons of 3 fresh solvent, dissolving the slurried solids by heating, coolingto crystallize, performing preliminary laboratory filtration; etc. as with the stage above.
:1. Store the filtrate from stage 3 in a storage; tank preparatory for the by-pass feature which, w lbe eg plained below.
FILTER STAGE 1 AND SET UP STAGE 2 OF NEXT ROW 11. Pump three thousand gallonsof fresh solvent into the filter cake receiver.
b. Filter stage 1, receiving thecake inthe fresh-sol vent.
c. Set up stage 2 of the next row by pumping the slurry.- to a stage tank, dissolving, crystallizing, etc. asabover FILTER STAGE -1 AND SET'UP'STAGE" 0 OF NEXT ROW a. Pump stage 1 filtrateto the filter cake receiver.
b. Filter stage l, receiving the cakein the stage 1 filtrate.
c. Set up stage 0 by pumping the slurrie'd' cake to a stage tank, distilling to adjust the concentration of solids to fall within the range previously described fol stripping- Determine water content and cool the slurry to an intermediate temperature of about 55 degrees centigrade; add the requisiteamountof Water toachieve the-desired-in" crease in ,8 value; stir the solution for aboutoneshalfy hour to assure solution of the added water; cool..the; stirred solution to about twenty degrees centigradetm crystallize a portion of the dissolved sterols; carry, out? preliminary filtration, determine the E value, and. adjust: the temperature of the slurry accordingly.
FILTER STAGE -3 AND SET UP STAGE 2 OF NEXT now a. Pump stage -.-l filtrate to the filter cake receiven,
b. Filter stage -3, receiving the cake in the stage --l filtrate.
c. Set up stage 2 by'distilling, preliminary cooling, adding water, and further cooling, as in stage 0'.
d. Distill stage 3 filtrate to recover the azeotropesol vent, and save the residue for further recovery of sterols present.
The above operations complete the filtration steps of the upper row of stages, leaving the lower row of stagesto be filtered. The lower row is treated as follows.
FILTER STAGE G (NO SET UP) a. Filter a major proportion of stage 6 onthefiltcl'. press; dry the cake as stigmasterol product. Leave the1 remainder of the slurry unfiltered in the stage tank, to be used as reflux to stage 5 of the succeeding row.
FILTER STAGE 4 AND SET UP STAGE 5 OF NEXT ROW a. Pump stage 6 filtrate tothe filter cake receiver.
b. Filter stage 4, receiving the cake in the stage. 6 filtrate.
c. Pump the slurry to the stage tank and combine, with; refiuxedslurry from the stage 6 filtration. Add solvent,; if necessary, to give desired solvent/solids ratio; heat; to dissolve, cool to crystallize, etc. as for, the setuprof stage 6 above.
FILTER STAGE 2 AND SET UP STAGE;
3 OF NEXT ROW a. Pump stage 4 filtratetothe filter cake;receiver l b. Filter stage 2, receiving the cake in the stage 4 filtrate.
0. Pump the slurry to stage tank and set up stage 3 of the next row as with stage above.
FILTER STAGE 0 AND SET UP STAGE 1 OF NEXT ROW a. Pump stage 2 filtrate to the filter cake receiver.
b. Filter stage 0, receiving the cake in the stage 2 filtrate.
- 0. Set up stage 1 by the following procedure. This includes the by-pass feature of this invention.
(1) Pump the slurry from the filter cake receiver to the stage tank.
(2) Heat to dissolve; distill to remove water from the solution. I
(3) Dissolve six thousand pounds of feed sterols in 2 300 gallons of fresh solvent, add fifty pounds of filter aid for clarification purposes, distill to remove water, filter, and add to the solution in the stage tank.
(4) Pump stage 3 filtrate (from storage) into the stage tank, cool entire mixture to crystallize, carry out prelimina'ry' filtration, etc., and complete set up as for stage 6 above.
FILTER STAGE -2 AND SET UP STAGE -1 OF NEXT RO\V 'a. Pump stage 0 filtrate to the filter cake receiver.
b. Filter stage -2, receiving the cake in the stage 0 filtrate.
0. Set up stage 1 by pumping the slurry to a stage tank, distilling to adjust the concentration of solids, and stripping the resulting solution as described above for stage 0.
, SET UP STAGE 3 OF NEXT ROW a. Pump stage -2 filtrate to stage tank. b. Strip as described for stage 0.
The foregoing illustrative procedure is taken from a large-scale process for separating stigmasterol from a feed of mixed soy sterols, the entire process having been operated a sufiiciently long time so that steady state conditions prevail. As can be seen, the stigmasterol productis of extremely high quality, the yield is very high, and the stigmasterol content of the process residue is very low. The efficiency of stripping contributes materially to the two latter features, i.e., high overall yield of stigmasterol product and low stigmasterol content of the residue.
- The foregoing example, including Figure 3 of the drawings, discloses an'additional novel feature of this invention, i.e., the'by-pass feature, as more particularly illustrated in the by-passing of stage'3 filtrate (upper row) to stage 1 set up (third row, not shown). By this procedure, as can be seen from Figure 3, the stage 3 filtrate passes by stage 2 of the lower row where it would normally enter. Instead of stage 3 filtrate, fresh make-up solvent is added to stage 2. This illustrative by-pass is an embodiment of an improvement gained by manipulating the flow of materials in the stages of a process as described above, so as to increase surprisingly the efficiency of the overall operation. It is based upon our discovery of the relationship between the variables that exist in a system employing a mixture of sterols containing sigmasterol, e.g., soy sterols, when employing as countercurrent selective separation solvent a mixture of a halogenated lower aliphatic hydrocarbon and a lower aliphatic hydro carbon, particularly the azeotrope of ethylene dichloride and n-heptane. It relates particularly to controlling the flow of solvent, and by-pass thereof, in a stabilized countercurrent system in such a manner that fewer enriching stages are required to produce an equivalent or better yield of equivalent or better quality stigmasterol product.
When the process as described herein has come to steady state conditions, we have found that a given variation in the E value results in a variation in yield of enriched stigmasterol cake of a given predetermined quality. We have discovered that the variation in over- .14... all yield which responds to a given variation in E, value is quite different at different stages. In other Words, the sensitivity of the overall yield to E variations varies from stage to stage. For example, a variation in E value at stage 1 will normally result in a much greater yield difference for a given quality final stigmasterol product than will result from the same variation in E value at stage 6. This sensitivity of the overall yield to E variations is an unique result of the physical relationships between materials (material balances) and the number andv arrangement of stages in the process. We have found that this uniqueness can be utilized advantageously to increase the overall yield of stigmasterol. This is done by bypassing the filtrates obtained from one or more of the first four enriching stages, i.e., stages 1, 2, 3 or 4 of any row, around the succeeding row, and entering said filtrates into stages 1, 0, 1 or 2, respectively, of the next succeeding row. When such a filtrate is by-passed in, one Or more of these manners, it is possible to operate the process at a maximum value of E without serious impairment of the quality of the final stigmasterol product.
Illustratively, the use of stage 3 to stage 1 by-pass by manipulation such as described above, altords the production of stigmasterol product of 90.8 percent average quality, using six enriching stages and two stripping stages, with an overall stigmasterol yield of 65.3 percent. Under otherwise comparable conditions, but without bypass, production of 90.1 percent quality stigmasterol product requires eight enriching stages and two stripping stages with an overall yield of 52.4 percent.
Instead of by-passing stage 3 to 1 as is illustrated in Figure 3, it is likewise feasible as noted above to by-pass stage 4 to stage 2, stage 2 to stage 0, or stage 1 to stage -1. The two stages involved in the by-passing of a particular filtrate can be determined by observing the quality of materials moving through the system. The by-pass points are selected so as to obviate mixingstreams containing sterols having markedly unequal stigmasterol content. It is feasible moreover to by-pass the filtrate around more than one stage, if necessary, to combine it with a cake of similar stigmasterol content.
It is to be understood that the invention is not to be limited to the exact details of operation or exact materials shown and described, as obvious modifications and equivalents will be apparent to one skilled in the art, and
the invention is therefore to be limited only by the scope of the appended claims.
We claim:
p 1. In a process for the separation and purification of stigmasterol and sitosterols by the extraction of sito-' sterols from a starting solid stigmasterol and sitosterols mixture consisting essentially of stigmasterol and sitosterols which comprises contacting the starting solid stigmasterol and sitosterols mixture with a selective organic solvent having the following characteristics; 1) a greater solvent aflinity for the siteosterols as determined on a test portion of said starting solid stigmasterol and sitosterols mixture by employing a volume of the organic solvent which dissolves approximately one-half of the solids of the test portion of the said starting solid stigmasterol and sitosterols mixture, and (2) a relative distribution coeflicient (18) in said test greater than 1.5, said relative distribution coefficient (5) being determined according to the formula:
wherein S is the stigmasterol content in percent of the undissolved solids, NS is the non-stigmasterol content in percent of the undissolved solids (by difference), S is the stigmasterol content in percent of the dissolved solids in the mother liquor, and NS is the non-stigmasterol content in percent of the dissolved solids in the mother liquor (by difference), to cause selective extraction of sense??- 15 the: .sitosterolsvfrom the .stigrnas terol, separating. hesolid material, phasewhich is. enriched. in,stigmasterol contentf iorn theprganic solvent. phase which is enrichedin :SltQS: t'ei-ols. content,. and continuin the extraction process. in; a countercurrent manner, passing said. solid material. phase through a series of enrichingstages to a stigmasa terol enriched end product, and passing said organic sglvent..phase through said series ofenrichingstages-im reverse. .olf fil'v and thencethrough; a .seriesvof, stripping.
stagesfrorn, each of which is obtained,.a.stigmasterol-..
poor solution and a cake. strippedtherefrom.containing.
stigmasterol, said solutions and said stripped cakes -travel-.
snfii'cient to increasejhe 13 value oflsaid selective. oi'gfautiev solventjn said stage.
2,-..Th8..process of claiml wherein the amountofiwater added is from, about. 2 to about. 3 moles, per. molevofstigmasterol in the first stripping stage, from about}. to.
aboutA moles. per. mole. of stigmasterol in. the second s ripping stage andfrom. about 2. to; about 6 moles permole. of, stigmasterol 1 in the. third stripping. stage.
3,...The process of claim 1 wherein the starting solid. sti'g nesterol and sitosterols mixtureis. amixture of soy. steiiols. and theselective organic. solvent is the. azeotrope;
ofimheptane and-ethylene dichloride.
4. A.. process for the. separation and purification. of stigmasterol and. sitosterols by the extractionof. sitesterolsfrom. a starting solid stigmasterol and, sitosterols mixture consisting essentially of stigmasterol and sitos-.
tGIOlS. which comprises. contacting the starting solid stigmasterol and sitosterols mixture with a selective organic solvent having the following characteristics; (1) a greater solvent affinity. for the sitosterols asdetermined on..a. test portion of said starting solid stigmasterol and.
sitosterols mixture by employing a volume of the organic solvent which dissolves approximately one-half of the. solidsof the test portion of the said starting, solid stigmasterol and sitosterols mixture, and.( 2)- a relative distribution coefiicient (B) in said test. greater than; 1.5,
said relative distribution coefiicient I (B). being, determined accordingtothe formula; 1 B= il} N ex S ml in which process said selective organic solvent passes through a. series of stages wherein dissolved sterols including stigmasterol are stripped therefrom, and between nd. tw moles f .wate P r, mole. of. stigmastcrol present is added to at least one of the group consisting of the first two enriching. stages andthestrippingstages, thereby to increase said fivalue. i l
5. The process of claim 4 wherein the amount of Water added is from-about 2 to-.about' 3' moles per'mole of stigmasterol in the first strippingstage, from about 2 to about 4 moles per mole of .stigmasterol' in the, second stripping stage and from about'2to about 6 moles per. mole of stigmasterol in the third stripping stage.
6. The processof claim 4 wherein the starting solid stigmasterol and sitosterols mixture is a mixtureiofsoy sterols.
7. The process of claim 4 wherein the organic solvent is the azeotrope of n-heptane and ethylene dichloride.
8. In a countercurrent selective solvent separation of stigmasterol from a mixtnre of sterols containing stig; masterol'by extraction with an organicsolvent compris ing a mixture of ahalogenated lower aliphatic hydro a direction opposite-to; the, -.dire cti.on of said' cakes, the improvement which comprises by-passing at least one of said organic solvent phases around atleast one of said cakes in such a' manner as to substantially match the, stigmastero] content of the solids dissolved in said organic-- sol-vent phases with the stigrnasterol content ofjs'aid. cakes to be extracted thereby.
9. The process of claim 8'wherein the forwardly'pass ing cakes and the countercurrently passing organic sol'-' vent phases are mixed in a series of stages: thereby to produce a corresponding series.=o.f; stigmasterol-containing cakes and organic solvent; phases. generally POOrerJin stigmasterol than said cakesandincluding-atleastsix stages of enrichment ofsaid cakes-in stigmasterol, and wherein the by-passing of-organic. solventphases is car-:
riedoutin the first four of-said stages of enrichment.
10. The. process of claim:9 inwhich the. mixtureof: sterols is amixture of soy sterols and the organic solvent:
is; the azeotropeofn-heptaneand ethylene dichloride.
References Cited in the, file of-thi s;patent; UNITED STATES PATENTS 2,730,536. Feeney ,.,Jan. 10, 1956.- 2..835,6.82 Steiner et al May 20, 1958. 2,839,544 Greineret .al June. 17, 1958' UNITED STATES PATENT OFFICE CERTIFICATE OF CORRECTION Patent Nos 2,905,677 September 22, 1959 Glen A. Fevig et al.2
It is hereby certified that error appears in the -printed specification of the above numbered patent requiring correction and that the said Letters Patent should read as corrected below.
Column 3, line 30, for "of non-stigmasterol" read of stigmasterol-- column '7, line 33, for "stake" read stage column 8, lines 16 and l? for "use of E values" read use of low E values column ll, line 18 Table V, second column thereof, last item, for "4 71" read 4701 Signed and sealed this 15th day of March 1960.,
(SEAL) Attest:
KARL AXLINE ROBERT c. WATSON Attesting Officer Commissioner of Patents

Claims (1)

1. IN A PROCESS FOR THE SEPARATION AND PURIFICATION OF STIGMASTEROL AND SITOSTEROLS BY THE EXTRACTION OF SITOSTEROLS FROM A STARTING SOLID STIGMASTEROL AND SITOSTEROLS MIXTURE CONSISTING ESSENTIALLY OF STIGMASTEROL AND SITOSTEROLS WHICH COMPRISES CONTACTING THE STARTING SOLID STIGMASTEROL AND SITOSTEROLS MIXTURE WITH A SELECTIVE ORGANIC SOLVENT HAAVING THE FOLLOWING CHARACTERISTIC; (1) A GREATER SOLVENT AFFINITY FOR THE SITEISTEROLS AS DETERMINED ON A TEST PORTION OF SAID STARTING SOLID STIGMASTEROL AND SITOSTEROLS MIXTURE BY EMPLOYING A VOLUME OF THE ORGANIC SOLVENT WHICH DISSOLVES APPROXIMATELY ONE-HALF OF THE SOLIDS OF THE TEST PORTION OF THE SAID STARTING SOLID STIGMASTEROL AND SITOSTEROLS MIXTURE, AND (2) A RELATIVE DISTRIBUTION COEFFICIENT (!) IN SAID TEST GREATER THAN 1.5, SAID RELATIVE DISTRIBUTION COEFFICIENT (B) BEING DETERMINED ACCORDING TO THE FORMULA:
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Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3153054A (en) * 1962-03-20 1964-10-13 Eastman Kodak Co Process for separating tocopherols and sterols from deodorizer sludge and the like
US3153055A (en) * 1962-03-20 1964-10-13 Eastman Kodak Co Process for separating tocopherols and sterols from deodorizer sludge and the like
US3526647A (en) * 1968-07-10 1970-09-01 Malmstrom Chem Corp Process for producing wool wax alcohols and fatty acids
US3965131A (en) * 1974-01-25 1976-06-22 Schering Aktiengesellschaft Process for the purification of crude chenodeoxycholic acid
US4549990A (en) * 1982-05-14 1985-10-29 Societe Dite: Exsymol S.A.M. Manufacture of non-saponifiable compounds from natural substances and the resulting products

Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2730536A (en) * 1952-05-01 1956-01-10 Pfizer & Co C Recovery of ergosterol
US2835682A (en) * 1955-08-08 1958-05-20 Swift & Co Sterol recovery process
US2839544A (en) * 1956-09-04 1958-06-17 Upjohn Co Countercurrent extraction of steroids

Patent Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2730536A (en) * 1952-05-01 1956-01-10 Pfizer & Co C Recovery of ergosterol
US2835682A (en) * 1955-08-08 1958-05-20 Swift & Co Sterol recovery process
US2839544A (en) * 1956-09-04 1958-06-17 Upjohn Co Countercurrent extraction of steroids

Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3153054A (en) * 1962-03-20 1964-10-13 Eastman Kodak Co Process for separating tocopherols and sterols from deodorizer sludge and the like
US3153055A (en) * 1962-03-20 1964-10-13 Eastman Kodak Co Process for separating tocopherols and sterols from deodorizer sludge and the like
US3526647A (en) * 1968-07-10 1970-09-01 Malmstrom Chem Corp Process for producing wool wax alcohols and fatty acids
US3965131A (en) * 1974-01-25 1976-06-22 Schering Aktiengesellschaft Process for the purification of crude chenodeoxycholic acid
US4549990A (en) * 1982-05-14 1985-10-29 Societe Dite: Exsymol S.A.M. Manufacture of non-saponifiable compounds from natural substances and the resulting products

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